Overview

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1.PrepareCells:

1.1   Foradherentcells:Platecellsovernightingrowthmediumat10,000to40,000cells/well/90µLfor96-wellplatesor2,500to10,000cells/well/20µLfor384-wellplates.

1.2   Fornon-adherentcells:CentrifugethecellsfromtheculturemediumandthensUSPendthecellpelletsinculturemediumat50,000-100,000cells/well/90µLfor96-wellpoly-Dlysineplatesor10,000-25,000cells/well/20µLfor384-wellpoly-Dlysineplates.Centrifugetheplatesat800rpmfor2minuteswithbrakeoffpriortotheexperiment.

Note:Eachcelllineshouldbeevaluatedonanindividualbasistodeterminetheoptimalcelldensity.

2.Prepare10XTrackIt™Redstainsolution:

Dilute500XTrackIt™RedDMSOstocksolution(ComponentA)intoAssayBuffer(ComponentB)tomakea10 to25XTrackIt™Redworkingsolution.Theworkingsolutionshouldbepreparedenoughforallthewellsat10μL/wellwiththeappropriateconcentration.Forexample,togeta1XfinalconcentrationofTrackIt™Redforone96-wellmicroplate,dilute20μLoftheTrackIt™RedDMSOstocksolutioninto1mLofAssayBuffer(ComponentB)tomake1mLof10XTrackIt™Redworkingsolution.

Note1:TheunusedportionoftheTrackIt™Redstocksolutionshouldbestoredat-20^oC.Avoidrepeatedfreeze/thawcycles.

Note2:ThefinalconcentrationoftheTrackIt™Redworkingsolutionshouldbeempiricallydeterminedfordifferentcelltypesand/orexperimentalconditions.Itisrecommendedtotestattheconcentrationsthatareatleastoveratenfoldrange

3.Stainthecells:

3.1   Tothecellwellsadd10XTrackIt™Redworkingsolution(fromStep2)whichshouldbeequalto1/10ofthevolumeofcellculturemedium.Forexample,fora96-wellplate,add10µL/wellof10XTrackIt™Redworkingsolutionintothecells.

3.2   Incubatethecellsina37^oC,5%CO₂incubatorfor15minutesto1hour.

3.3   WashcellswithHanksand20mMHepesbuffer(HHBS)oranappropriatebuffer.

3.4   Fillthecellwellswithgrowthmedium.

3.5   AnalyzethecellsusingafluorescencemicroscopeorflowcytometerwithTexasRedfiltersets(Ex/Em=570/600nm).

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